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OPTIMISATION OF PROTOCOLS FOR DETECTION OF FREE
CHOLESTEROL AND NIEMANN-PICK TYPE C 1 AND 2 PROTEIN
Linda M. Scott
Biomedical Science
May 2010
School of Biological Sciences BMC, Uppsala University
Dublin Institute of Technology Department of Medical Biochemistry
Kevin Street and Microbiology
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ABSTRACT
The purpose of this project was to optimise the protocols for detection of free cholesterol
and NPC 1 and NPC 2 proteins. Paraffin embedded human and rat tissues, cellblocks and
cytospins of HepG2 and HeLa cells were used for immunohistochemistry to try out the
best antibody dilutions and unmasking method of the antigen. Adrenal tissue was used to
stain lipids with Filipin. The dilution that worked best for the NPC 1 was 1:150 and with
EDTA unmasking. For the NPC 2 the dilution 1:100 was optimal and with Citrate as
unmasking method. NPC 1 was highly expressed in ovary tissue, stomach epithelium,
HeLa cells and rat kidney and liver, while NPC 2 was highly expressed in neurons and
astrocytes in Alzheimer’s disease, seminiferous tubules in testis, neurons in intestine,
neurons in healthy brain tissue and HeLa cells. The cholesterol inducing chemical
U18666A was applied to HepG2 cells but no alteration in lipid staining was observed and
NPC protein expression was similar at all doses applied. Filipin staining worked well with
a concentration of 250µg/mL and Propidium Iodide with concentration 1mg/mL for nuclei
stain was optimised at 1:1000.The fixation of cells before lipid stain and
immunoperoxidase staining has to be evaluated further as the fixations used, 10% formalin
and acetone, had adverse effects on the antigen.
In this project methods were optimized for lipid and NPC protein staining for further
application in disease investigations.
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CONTENTS
TITLE PAGE .........................................................................................................................1
ABSTRACT ..........................................................................................................................2
CONTENTS ..........................................................................................................................3
ACKNOWLEDGEMENTS ..................................................................................................6
1. INTRODUCTION .............................................................................................................7
1.1 Cholesterol ...................................................................................................................7
1.1.1 Structure ......................................................................................................................7
1.1.2 Metabolism & Synthesis .............................................................................................7
1.1.3 Structural function .....................................................................................................9
1.1.4 Distribution ............................................................................................................... 10
1.1.5 Visualisation .............................................................................................................. 10
1.1.6 Atherosclerosis .......................................................................................................... 11
1.2 Niemann-Pick type C (NPC) proteins ................................................................. 12
1.2.1 NPC 1 ......................................................................................................................... 12
1.2.2 NPC 2 ......................................................................................................................... 13
1.2.3 Function ..................................................................................................................... 13
1.2.4 Associated diseases ................................................................................................... 14
1.2.5 Investigation of NPC proteins/Immunostaining .................................................... 15
1.3 Aim ............................................................................................................................... 16
2. MATERIALS AND METHODS .................................................................................... 17
2.1 Summary ...................................................................................................................... 17
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2.2 Cell culture – HeLa and HepG2 cells ........................................................................ 17
2.3.i Harvesting – HeLa cells ............................................................................................ 18
2.3.ii HepG2 cells – Exposure to U18666A experiment .................................................. 18
2.4 Cellblock preparation ................................................................................................. 19
2.5 Cytospin preparation .................................................................................................. 19
2.6 Sudan Black B protocol ............................................................................................... 19
2.7 Oil Red O protocol ....................................................................................................... 20
2.8 Filipin stain ................................................................................................................... 20
2.9 Immunoperoxidase staining ....................................................................................... 20
3. RESULT .......................................................................................................................... 22
3.1 Sudan Black B .............................................................................................................. 22
3.2 Oil Red O ...................................................................................................................... 22
3.3 Filipin stain ................................................................................................................... 23
3.4 Immunoperoxidase staining for NPC 1 and NPC 2 proteins .................................. 25
3.4.1 Normal and diseased tissues ....................................................................................... 25
3.4.2 HepG2 and HeLa cells ................................................................................................ 28
4. DISCUSSION .................................................................................................................. 31
4.1 Sudan Black B and Oil Red O .................................................................................... 31
4.2 Filipin stain ................................................................................................................... 31
4.3 Immunoperoxidase staining ....................................................................................... 32
4.4 Conclusion .................................................................................................................. 34
5. APPENDICES ................................................................................................................. 35
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5.1 Haematoxylin and Eosin – paraffin sections ............................................................. 35
5.1.1 Material H & E-stain – paraffin sections .................................................................... 35
5.2 Haematoxylin and Eosin stain – frozen sections ....................................................... 35
5.2.1 Material H&E-stain – frozen sections ........................................................................ 36
5.3 Cell culture ................................................................................................................... 36
5.4.i Harvesting – HeLa cells ............................................................................................ 36
5.4.ii HepG2 cells – Exposure to U18666A experiment .................................................. 36
5.5 Cellblock preparation ................................................................................................. 37
5.6 Sudan Black B protocol ............................................................................................... 37
5.7 Oil Red O protocol ....................................................................................................... 38
5.8 Filipin stain ................................................................................................................... 38
5.9 Immunoperoxidase staining ....................................................................................... 38
6. REFERENCES ................................................................................................................ 40
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ACKNOWLEDGEMENTS
I would like to thank my supervisor Dr. Helen Lambkin for all her guidance and help
throughout this project. I have learned a great deal from her.
I would also like to send a big thank you to Kathleen Flynn, laboratory technician, for all
her help with materials and solutions that I needed on this project.
Finally I would like to thank my parents for making this stay in Dublin a possibility.
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1. INTRODUCTION
1.1 Cholesterol
Cholesterol is produced in the body by the liver (Kruit et al., 2006). The production of
cholesterol occurs mostly during the night time (www.sund.nu). Cholesterol is present in
tissues and plasma as free cholesterol or as cholesterol esters which is the storage form of
cholesterol (Murray et al., 2009).
1.1.1 Structure
Cholesterol belongs to the family of steroids (Thabrew & Ayling, 2001). The cholesterol
structure consists of three six-membered rings and one five-membered ring (Campbell &
Farrell, 2009) which is the basic structure of all steroids. Cholesterol has a single hydroxyl
group which makes the cholesterol molecule very hydrophobic (Fig. 1.1) (Campbell &
Farrell, 2009).
Figure 1.1 Structure of the cholesterol molecule can be seen at
http://www.papermag.com/blogs/Cholesterol2.gif
1.1.2 Metabolism & Synthesis
The biosynthesis of cholesterol may be divided into five steps (Fig. 1.2) (Murray et al.,
2009):
In the first step two molecules of Acetyl-CoA are converted by Thiolase to be
Acetoacetyl-CoA. This is then acted on HMG-CoA synthase to make HMG-CoA (3-
hydroxy-3-methylglutaryl-CoA). HMG-CoA gets reduced to Mevalonate by NADPH
catalyzed by HMG-CoA reductase.
In step two mevalonate is phosphorylated by ATP by three kinases. Then after
decarboxylation isopentenyl diphosphate is formed.
In step three isopentenyl diphosphate is isomerized as the double bound shift and form
dimethylallyl diphosphate. It is then condensed with another molecule of isopentenyl
diphosphate and forms the ten-carbon intermediate geranyl diphosphate. Another
condensation with isopentenyl diphosphate forms farnesyl diphosphate. Squalene is then
formed by two molecules of farnesyl diphosphate that condense at the diphosphate end.
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In step four squalene is converted to squalene 2,3-epoxide by squalene epoxidase.
Oxidosqualene:lanosterol cyclase transfer the methyl group on C14 to C13 as cyclization
occours and forms Lanosterol.
The last fifth step takes place in the membranes of the endoplasmatic reticulum. The
methyl groups are removed and forms 14-desmethyl and then zymosterol. The double bond
in the cholesterol molecule is placed at C8-C9 at first but is then moved to C5-C6 and forms
desmosterol. The double bond on the side chain is reduced and cholesterol is produced.
Figure 1.2 A schematic illustration of the cholesterol synthesis can be seen at
http://www.reactome.org/figures/cholesterol_biosynthesis.jpg
We also get cholesterol from the food we eat, the exogenous pathway, and it is absorbed by
the intestine (Kruit et al., 2006). It gets transported to the liver and other tissues in
chylomicrons (Kruit et al., 2006) which are a type of lipoprotein produced in the small
intestine (www.wikipedia.org).
To uphold the cholesterol metabolism the liver compensates a diet consisting of high
cholesterol intake by making less of it (www.wikipedia.org).
Free cholesterol cannot be transported in the blood on its own since it is insoluble in
water (Gurr et al., 2002). A transporter, lipoprotein, is required. The two common ones are
LDL, low density lipoprotein, and HDL, high density lipoprotein.
LDL transports the cholesterol from the liver to the rest of the body (Campbell &
Farrell, 2009). LDL is made by the liver as VLDL at first. After obtaining molecules from
HDL it becomes a mature VLDL and then turned into IDL, intermediate density
lipoprotein, by lipoprotein lipase. It is then converted to LDL by transferring
triacylglycerol or phospholipids to HDL and cholesteryl esters are transferred from HDL to
IDL (Thabrew & Ayling, 2001). LDL contains protein, triacylglycerol, cholesterol,
phospholipids and apoprotein B (Gurr et al., 2002). On the cell surface there are LDL
receptors. LDL binds to the receptors and the complex goes into the cell by endocytosis
(Thabrew & Ayling, 2001). The receptor then goes back to the surface while the LDL
particle ends up in the lysosomes where they are degraded (Thabrew & Ayling, 2001). The
cholesterol esters are hydrolyzed to free cholesterol and fatty acids (Thabrew & Ayling,
2001). The free cholesterol can be used directly by incorporation into the cell membrane,
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or it can be stored as cholesteryl esters catalyzed by ACAT, acyl-CoA:cholesterol
acyltransferase (Thabrew & Ayling, 2001).
To uphold the metabolism and to prevent too much free cholesterol accumulation in the
cell there is a feedback system that protects the cell from getting over loaded with
cholesterol (Vance & Vance, 2004). First HMG-CoA synthase and HMG-CoA reductase is
suppressed. Then cholesterol activates ACAT (Acyl-coenzyme A:cholesterol
acyltransferase) which makes the cell able to store excess cholesterol in re-esterified form.
Then the LDL receptor synthesis is suppressed so the LDL entry into the cell decreases
(Vance & Vance, 2004). This can on the other hand lead to increase of LDL particles in the
blood stream which can lead to plaque in the artery walls.
HDL, high density lipoprotein, is part of reverse cholesterol transport and transports
cholesterol back to the liver (Schmitz & Grandl, 2009). HDL is mainly derived from the
liver though a small amount can be synthesised by the intestine (Thabrew & Ayling, 2001).
It contains protein, cholesterol, phospholipids, tricylglycerol and apoproteins A, C, D and
E (Gurr et al., 2002). The cholesterol taken up by HDL will either be eliminated from the
body as bile acid or reused (Schmitz & Grandl, 2009).
The two pathways for cholesterol synthesis, liver synthesis and absorption by the
intestine, maintain the metabolism of cholesterol along with biliary excretion (Yu et al.,
2006).
Biliary excretion is the body’s way to get rid of excess cholesterol. Cholesterol is
converted into bile acid by the liver and secreted from the gallbladder into the small
intestine (Vance & Vance, 2004).
1.1.3 Structural function
Though many may refer to cholesterol as something bad it is absolutely necessary for the
body.
Cholesterol is a necessary component for the membranes of the cells. It establishes
membrane permeability and fluidity (Mouritsen et al., 2004).
It works as isolating material around the nerve cells, in the myelin (Verheijen et al.,
2009).
Cholesterol is the precursor for the production of certain hormones in the body such as
testosterone, oestrogen and cortisol (Gurr et al., 2002).
Bile acid that is synthesised in the liver comes from cholesterol and is used to digest fat
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(Staels et al., 2009).
Vitamin D which is a fat soluble vitamin is made from 7-dehydrocholesterol, a precursor
to cholesterol (www.wikipedia.org). It is made in the skin when exposed to sunlight
(www.wikipedia.org). Vitamin D increase synthesis of a Ca2+
-binding protein which
increase the uptake of calcium in the intestines (Campbell & Farrell, 2009).
1.1.4 Distribution
Cholesterol is located in most places in the body, in all cell membranes. It is located in the
adrenals where the hormones cortisol and aldosterone are synthesised
(www.wikipedia.org).
The ovary and testis contain cholesterol due to the synthesis of sex hormone
(www.wikipedia.org).
It is located in the myelin that surrounds the nerve cells (Verheijen et al., 2009).
1.1.5 Visualisation
In 1924 Schultz adapted a reaction to visualize cholesterol in tissues (Bancroft & Stevens,
1990). The method was to let the tissue sections oxidise in air with iron alum and followed
by treatment with a sulphuric-acetic acid mixture that gave free and esterified cholesterol a
blue colour (Bancroft & Stevens, 1990). In 1961 Adams used a perchloric acid-
naphthoquinone (PAN) method. It was more sensitive, had precision and preserved the
tissues better (Bancroft & Stevens, 1990). Perchloric acid condense cholesterol to cholesta-
3:5-diene. This is then converted to a blue colour by 1:2 naphthoquinone (Bancroft &
Stevens, 1990).
To visualise cholesterol and lipids in tissues histochemically, by microscopy, there are
some common stains used.
Oil Red O (Haimovici et al., 2001) and Sudan Black B (Marounek et al., 2007) are used
on frozen tissue and are the two basic staining methods for visualisation of lipids. There
are different kinds of Sudan dyes but the most sensitive and versatile one is the Sudan
Black B, introduced in 1935 (Bancroft & Stevens, 1990). To be able to penetrate fats the
Sudans and Oil Red O have to be dissolved in organic solvents. The solvent though should
be sufficiently aqueous to avoid extractions of the lipids on their own (Bancroft & Stevens,
1990). The solvent usually used for Oil Red O is 60% isopropanol and for the Sudan Black
B 70% ethanol (Bancroft & Stevens, 1990). The Sudan methods fail to stain some lipids as
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they tend to dissolve in the dye (Bayliss, 1981). To prevent that, the tissues can be pre-
treated with bromine which makes the lipids more stabilised (Bayliss, 1981). As the names
suggest, the colours of the tissues (lipids) will appear red with the Oil Red O staining and
black with the Sudan Black B stain.
Filipin is a fluorescence method and is used to visualize free cholesterol (Yu et al.
2006). The detection of the Filipin stain is in the UV range, 360-460nm
(www.lipidomicnet.org). The colour will appear blue when viewed in fluorescence
microscope (Fig. 1.3). Filipin was isolated by chemists at the Upjohn company in 1955
from the mycelium and culture filtrates of an actinomycete, Streptomyces filipinensis
(www.wikipedia.org) and is a polyene antibiotic (Brock, 1956). It was discovered in a soil
sample that was collected in the Philippine Islands (www.wikipedia.org). The
identification of the Filipin as a polyene macrolide was based on its characteristic UV-Vis
(Ultraviolet-visible spectroscopy) and IR (Infrared) spectra (www.wikipedia.org). Filipin
III is the major component in Filipin (www.sigmaaldrich.com) and it has a strong affinity
to cholesterol and therefore very useful for visualization of cholesterol in cell membranes
(Volpon & Lancelin, 2000), often in relation with the study and diagnosis of Niemann-Pick
type C disease (www.wikipedia.org).
Figure 1.3 Filipin stain can be seen at
http://farm4.static.flickr.com/3183/2611112097_8131650aa6_o.jpg
1.1.6 Atherosclerosis
This condition results in development of plaques in the arteries (Fig. 1.4). The plaque will
cause the blood flow to the heart and other parts of the body to decrease which can
eventually lead to for example a heart attack or a stroke.
The cause of plaque can be due to the increase of LDL in the blood stream and because
the LDL oxidizes (www.wikipedia.org). When the oxidized LDL accumulates in the artery
wall an inflammatory reaction starts (Berliner et al., 1995) and an increase of macrophages
infiltration appears (Holvoet et al., 2008). They feed on the LDL-particles which makes
them filled with fatty droplets and known as foam cells. The macrophages cannot process
the oxidized LDL and will eventually rupture which will release the LDL in the artery wall
and lead to more infiltration of macrophages (www.wikipedia.org). All this will eventually
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promote growth of plaque and a fibrous cap forms over the lipid core as a result from the
death of foam cells (Vance & Vance, 2004) which seals off the core from the blood. Foam
cells secrete digesting matrix molecules which weaken the cap and if it ruptures tissue
factors from the macrophages (foam cells) interact with clot-promoting elements in the
blood and leads to a clot in the artery (Campbell & Farrell, 2009).
Figure 1.4 A picture of plaque can be seen at http://www.web-
books.com/eLibrary/Medicine/Cardiovascular/Images/Athero.gif
1.2 Niemann-Pick type C (NPC)
The Niemann-Pick type C 1 (NPC 1) gene was discovered by scientists at the National
Institutes of Health in 1997 (Carstea et al., 1997) and the NPC 2 gene was discovered in
2000 (Naureckiene, 2000).
The gene for NPC 1 is located on chromosome 18 between positions 11 and 12 (nih.gov)
(Fig. 1.5.a). The NPC 2 gene is located on chromosome 14 at position 24.3 (nih.gov) (Fig.
1.5.b).
Figure 1.5.a and Figure 1.5.b Location of the NPC 1and NPC 2 genes can be seen at
http://ghr.nlm.nih.gov/gene=npc1, http://ghr.nlm.nih.gov/gene=npc2
1.2.1 NPC 1
NPC 1 protein is located in the membrane of late endosomes in the cells (Chang, 2005)
(Fig. 1.6). It is also transiently associated with lysosomes and Golgi (Chang, 2005).
It spans more than 47kb (Storch & Xu, 2009). It contains 25 exons with sizes from 74 to
788 nucleotides and introns with sizes between 0,097 and 7kb (Storch & Xu, 2009). The
protein consists of 1278 amino acids (Goldman & Krise, 2010). It has 13 putative
transmembrane helices, three large hydrophilic domains that project into the lumen of the
endosomes and lysosomes as well as four small luminal loops, six small cytoplasmic loops
and a cytoplasmic tail (Storch & Xu, 2009). A sterol-sensing domain (SSD) is located
between the third and seventh transmembrane domains and is needed for the NPC 1 to
mediate sterol binding (Chang et al., 2005).
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Over 200 mutations have been identified in the NPC 1 gene that causes Niemann-Pick
type C disease (Storch & Xu, 2009).
Figure 1.6 Picture of NPC 1 located in the membrane can be seen at
http://www.uoguelph.ca/~fsharom/research/images/npc1+2function.png
1.2.2 NPC 2
NPC 2 is a protein with 132 amino acids (Ory, 2004) and is 13.5kb long (Storch & Xu,
2009). It is a soluble protein located in the lysosomes in the cells (Goldman & Krise,
2010). It contains five exons in sizes from 78 to 342bp (Storch & Xu, 2009). The crystal
structure shows an immunoglobulin-like β-sandwich fold consisting of seven β-strands
arranged in two β-sheets (Storch & Xu, 2009) (Fig 1.7). The structure contains three
potential N-glycosylation sites at positions 19, 39 and 116 and is composed in different
isoforms and all the forms are able to bind cholesterol (Storch & Xu, 2009). The crystal
structure shows that the protein has three small hydrophobic cavities that may be a binding
site for cholesterol (Chang et al., 2005).
More than 15 mutations that cause Niemann-Pick type C disease have been found in the
NPC 2 gene (nih.gov).
Figure 1.7 Structure of the NPC 2 protein can be seen at
http://stock.cabm.rutgers.edu/coord/NPC2/npc2.gif
1.2.3 Function
NPC 1 is required for the egress of cholesterol and other lipids from the endosomal
pathway (Kulinski & Vance, 2007). The movement of free cholesterol out of the late
endosomes or lysosomes is a main task for NPC 1 (Ishibashi et al., 2008), the protein
transports LDL to late endosomal/lysosomal compartments where the LDL is hydrolyzed
and releases its free cholesterol (www.proteinatlas.org).
NPC 2 is a high affinity cholesterol binding protein (Heo et al., 2006). It binds
cholesterol with a 1:1 stoichiometry and submicromolar affinity (Ory, 2004). It uses
mannose 6-phosphate marker for targeting to late endosomes (Chang et al., 2005). Studies
have shown that NPC 2 can transfer cholesterol to the membrane very quickly (Storch &
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Xu, 2009). The NPC 2 gene encodes a lipid recognition domain in the NPC 2 protein. This
function may be involved in the regulating of cholesterol transport through the late
endosomal/lysosomal system (www.proteinatlas.org).
A model of how the egress of cholesterol from lysosomes can take place with
cholesterol from LDL that binds to the NPC 2 protein and gets transferred in the lysosomes
to the NPC 1 protein in the lysosome membrane is shown in Fig. 1.8 (Kwon et al., 2009).
There is still more though to find out about these proteins since the exact function of
them is not yet fully established.
Figure 1.8 The transfer of cholesterol in the lysosome by NPC 1 and NPC 2 proteins can
be seen in the article by Kwon et al., 2009 via PubMed
1.2.4 Associated diseases
Niemann-Pick type C disease is a fatal neurodegenerative disease that occurs in childhood
(Phillips et al., 2008). It is a genetic disease that is autosomal recessive and is caused by a
mutation in one of the proteins NPC 1 and NPC 2 (Chang et al., 2005). Mutations in NPC1
stands for 95% of the cases involving Niemann-Pick type C disease (Reid et al., 2004). The
characteristic of this disease is the accumulation of cholesterol in the late endosomes,
lysosomes and tissues such as liver, spleen and brain (Ishibashi et al., 2009; Frolov et al.,
2003). Symptoms for Niemann-Pick type C disease are ataxia, dementia, vertical
supranuclear gaze palsy, dystonia, seizures, dysarthria and dysphagia (Patterson M, 2000).
Mutations in the NPC 1 and NPC 2 genes causes a disturbance in cholesterol homeostasis
(Goldman & Krise, 2009).
Liver cell death can be a result of cholesterol accumulation caused by a mutation in the
NPC 1 gene (Beltroy et al., 2005). This because the liver is taking care of the circulating
cholesterol from the plasma and the cholesterol gets trapped in the late endosomal and
lysosomal compartment because of the mutation (Beltroy et al., 2005).
Drugs such as antipsychotic and antidepressant that are used for schizophrenia and
bipolar disorder have been proven to activate Sterol Regulatory Element-Binding Protein
(SREBP) transcription factors that control genes involved in cholesterol biosynthesis (Vik-
Mo et al., 2009). This affects the NPC 1 and NPC 2 proteins and can cause cholesterol
accumulation and disturbed myelin structure (Vik-Mo et al., 2009).
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Studies have shown that lack of NPC 1 in mice have effect on the retina (Claudepierre et
al., 2010). NPC 1 is concentrated in specific layers of the mouse retina and if the NPC 1
protein is absent it causes severe defects in retinal morphology such as impaired visual
function and up-regulation of proteins that mediate cellular cholesterol release in the retina
(Claudepierre et al., 2010).
NPC 2 has in a study shown that it is involved in pulmonary disease. A severe case of
alveolar lipoproteinosis was discovered (Bjurulf et al., 2008).
1.2.5 Investigation of NPC proteins/Immunostaining
Immunostaining is an antibody based method (www.wikipedia.org). Antibodies are a
commonly used tool in immunohistochemistry, IHC (Bordeaux et al., 2010). It is used to
detect a special protein, molecule or such, an antigen, in a sample to visualize in a light
microscope or in a fluorescence microscope (www.wikipedia.org).
To visualize the NPC 1 and NPC 2 proteins, antibodies are required. Sigma-Aldrich
provides antibodies for both NPC 1 and NPC 2 (www.sigmaaldrich.com). The antibodies
are made in rabbit and are specifically targeting human NPC proteins, Anti-NPC 1 and
Anti-NPC 2 (www.sigmaaldrich.com).
The two types of immunostaining that are commonly used are immunoperoxidase and
immunofluorescence.
The immunoperoxidase method uses an enzyme, peroxidase, to visualize the antigen in
question often a protein. When adding a substrate it reacts with the enzyme and catalyzes a
chemical reaction to produce a coloured product (www.wikipedia.org) that can be viewed
in a light microscope.
Immunofluorescence is often used when wanting to visualize a bio molecular antigen
(www.wikipedia.org). Instead of an enzyme a fluorescent label is used, a fluorophore
(www.wikipedia.org). After incubation it is ready to visualize the antigen in a fluorescence
microscope. One problem though with using a fluorescence label is that it bleaches
quickly. It is very important that the fluorescence is kept from light exposure for long
periods.
Parallels between Niemann-Pick type C disease (NPC) and Alzheimer’s disease (AD)
has been seen due to histopathological characteristics (Vance et al., 2005). Endosomal
abnormalities can be seen in both NPC and AD with accumulate cleaved APP (amyloid
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precursor protein) and Aβ40 and Aβ42, plaque (Koh & Cheung, 2006). A common thing
between the two diseases is that neurofibrillary tangles occur in the brain (Vance et al.,
2005).
1.3 Aim
The aim for this project was to optimise the protocols for the detection of free cholesterol
and NPC 1 and NPC 2 proteins.
The protocols were first established on positive control tissues that were known to be
cholesterol rich. The right dilutions of antibodies and buffer for unmasking were
established before trying it out on cell lines. For this project HeLa cells and HepG2 cells
were used.
HeLa cells are a human immortal cell line from cervical cancer cells
(www.wikipedia.org).
HepG2 cells are a human liver carcinoma cell line, hepatocellular (www.wikipedia.org).
The HepG2 cells were treated with U18666A to trigger cholesterol accumulation.
U18666A is a cell permeable amphiphilic amino steroid that inhibits the intracellular
biosynthesis and transport of cholesterol (www.merck-chemicals.com).
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2. MATERIALS AND METHODS
2.1 Summary
Multiple tissue blocks were used during this project, which had been fixed in 4% formalin
and then processed to paraffin wax, available in paraffin blocks ready to use. A dissection
of a rat was performed during this project from which we took the brain and the adrenals as
lipid controls. Some of the brain was fixed in 4% formalin. The adrenals and the rest of the
brain were frozen in liquid nitrogen. The formalin fixed brain was processed to wax and
then paraffin embedded in blocks.
HeLa- and HepG2 cells were cultured in flasks and after harvesting cytospins and
cellblocks were prepared.
Immunoperoxidase staining was performed on the tissue sections, cellblocks and
cytospin preparation and fluorescence stain with Filipin III was performed on the frozen
adrenals and cytospins.
Paraffin tissues and cellblocks were also stained with Haematoxylin and Eosin (App. 5.1
and 5.1.1) for cell identification purposes. Rapid Haematoxylin and Eosin stains (App. 5.2
and 5.2.1) were used to check the histology of the frozen adrenals prior to lipid staining.
2.2 Cell culture – HeLa and HepG2 cells
The medium that was used was 500mL RPMI medium from Sigma (App. 5.3). 60mL
foetal calf serum, 5mL of 200mmol glutamine and 2mL of 10000 units/mL penicillin/
10000mg/mL streptomycin (App. 5.3) were added to the medium after defrosting them in a
37°C incubator for 30 min. Some of the mixed medium was poured into a 20mL sterile
universl container (Greiner bio-one) and defrosted HeLa and HepG2 cells were transferred
into the sterile universal container. 5mL of the medium was poured into a 25cm2 tissue
culture flask (Sarstedt). The sterile universal container containing the culture cells was
centrifuged at 1200rpm for 5 min at approximately 20°C. The medium was decanted and
cells resuspended in 5mL fresh medium and then poured into the tissue culture flask. The
flask was then placed in a 37°C, 5% CO2 incubator for three days before harvesting and
splitting the cells into new flasks.
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2.3.i Harvesting – HeLa cells
10mL trypsin (App. 5.4.i) was defrosted in a 37°C incubator for 30 min. Then equal
amount of EDTA/PBS (App. 5.4.i) was added to the trypsin. The medium in the cell flask
was decanted and 5mL of trypsin + EDTA/PBS was added for 1 min. The trypsin was
poured out and 5mL of new trypsin + EDTA/PBS was added and the flask placed in the
incubator for 15 min. The phase contrast microscope was used to verify that the cells were
free from the flask. The cell solution was poured into a sterile universal container (Greiner
bio-one) and equal amount of medium was added to neutralize the trypsin. The cells were
then centrifuged at 1500rpm for 10 min. The supernatant was then decanted and the cells
were resuspended in 5mL medium. 1mL each was then added into two new tissue culture
flasks, 75cm2, (Greiner bio-one) which contained 50mL medium. The flasks were placed
in the incubator at 37°C, 5% CO2.
2.3.ii HepG2 cells – Exposure to U18666A experiment
The same procedure was followed with the HepG2 cells. Ten 25cm2 tissue culture flasks
(Sarstedt) were used, marked from 1-10. After being in the incubator for two days,
100µg/mL U18666A (App. 5.4.ii) in different concentrations (Table 2.2) was added to the
flasks to accumulate the cholesterol in the cells. 5µL DMSO (dimethyl sulphoxide) was
added to all ten flasks to have the right conditions. Then 10µL of 100µg/mL working
solution U18666A was added to flasks 2 and 7, 20µL was added to flasks 3 and 8, 40µL
was added to flasks 4 and 9 and finally 60µL was added to flasks 5 and 10. This was to see
the differences in the expression of the NPC 1 and NPC 2 proteins.
Table 2.2 Concentrations of U18666A in cholesterol induction experiment on HepG2 cells.
Flask Amount of 100µg/mL U18666A Final concentration
1 and 6 - -
2 and 7 10µL 0.2µg/mL
3 and 8 20µL 0.4µg/mL
4 and 9 40µL 0.8µg/mL
5 and 10 60µL 1.2µg/mL
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2.4 Cellblock preparation
10mL trypsin (App. 5.5) was defrosted in 37C incubator for 30 min. Then equal amount of
EDTA/PBS (App. 5.5) was added to the trypsin. The medium in the cell flasks were
decanted and 5mL of trypsin + EDTA/PBS was added for 1 min. The trypsin was poured
out and 5mL of new trypsin + EDTA/PBS was added and the flasks placed in the incubator
for 15 min. A check in a phase contrast microscope was performed to see that the cells
were free from the flask. The cell solution was poured into a sterile universal container
(Greiner bio-one) and 5mL of medium was added to neutralize the trypsin. The sterile
universal containers containing the cells were then centrifuged at 1500rpm for 10 min. The
medium was poured off and 10% formalin (App. 5.5) was added and cells were fixed for
1h. The cells were then centrifuged again at 1500rpm for 10 min. The formalin was poured
off and 2% warm bacteriological agar (App. 5.5) was added and then centrifuged for 10
min at 1500rpm. The containers were placed in a fridge for 1h to let the agar solidify. Then
the agar was dislodged and 10% formalin was added for a few hours or overnight. The
formalin was poured off and pieces from the agar were cut and processed to wax with
Histokinette 2000 for 15h. The cellblocks were then embedded in paraffin.
This was done for both the HeLa and HepG2 cells.
2.5 Cytospin preparation
Labelled slides were placed in a clip device along with filter and funnel and then placed in
the centrifuge head. 3-6 drops of cell suspension (depending on cell yield) were added to
the funnels. The centrifuge head was then placed in the Shandon Cytospin centrifuge for 5
min at 1500rpm. The slides were air-dried, three were retained unfixed and three were
fixed in acetone for 5 min and then air dried, before wrapped in tin foil and placed in the
freezer, -80°C, for later staining.
2.6 Sudan Black B protocol
Frozen rat adrenal and cytospins of HepG2 cells were stained with Sudan Black B. The
slides were fixed in 10% formalin (App. 5.7) for 5 min and then rinsed in tap water. They
were then treated with 2.5% aqueous bromine (App. 5.7) for 30 min in fume hood because
of the toxicity. Slides are then rinsed in tap water and 0.5% sodium metabisulphite (App.
5.7) is placed on the slides for removal of excess bromine. Slides were washed in tap water
20
and rinsed in 70% ethanol (App. 5.7) for 1 min. Working solution of Sudan Black B (App.
5.7), filtered before use, was added to the slides for 8 min and then 70% ethanol to remove
extra stain, 2 min. Nuclei were then stained for 5 min with 0.2% Neutral Red (App. 5.7).
Slides were then washed in tap water and mounted with glycerine jelly (App. 5.7).
2.7 Oil Red O protocol
Frozen rat adrenal and cytospin with treated HepG2 cells were also stained for Oil Red O.
Slides were fixed in 10% formalin (App. 5.8) for 5 min, rinsed in distilled water and then
placed in a coplin jar with 60% isopropanol (App. 5.8) 3 min. Slides were then stained
with Oil Red O working solution (App. 5.8), filtered before use, for 15 min then washed in
60% isopropanol to clear background, 1 min. Slides were washed in tap water and nuclei
were stained with Mayer’s Haematoxylin 30 sec. Nuclei were blued in warm tap water and
mounted with glycerine jelly (App. 5.8).
2.8 Filipin stain
Frozen rat adrenal and cytospins were stained with the fluorescence method Filipin for
detection of free cholesterol. Slides were fixed in 3% formalin (App. 5.8) for 10 min and
then rinsed with PBS (App. 5.8) 3x2 min. They were then quenched with 1.5mg/mL
glycine in PBS (App. 5.8) 10 min. Filipin with the concentration of 250µg/mL (App. 5.8)
was added to the slides for 2h in the dark to prevent Filipin from fading. The slides were
then rinsed in PBS 3x2 min. Propidium Iodide (1mg/mL), for nuclei stain, with dilution
1:1000 were added for 5 min then glycerol (App. 5.8) was added to the slides and
mounted.
2.9 Immunoperoxidase staining
Tissues, cytospin and cellblocks were immunostained with antibodies NPC 1 and NPC 2
from Sigma-Aldrich. Concentration of NPC 1 is 0.33mg/mL and for NPC 2 0.07mg/mL.
The polyclonal antibodies are produced in rabbit by inserting a recombinant human
protein, Niemann-Pick C1 protein Precursor, PrEST protein (protein epitope signature tag)
(www.sigmaaldrich.com; www.wikipedia.org). A Vectastain ABC kit from Vector
Laboratories was used. The tissues were cut at 5µm and placed on APES (App. 5.9) and
the cellblocks at 7µm and placed on Superfrost slides (App. 5.9) and then left in the oven
for 1-1.5h at 60°C. After dewaxing, the slides were put in citrate or EDTA buffer (App.
21
5.9) and micro waved for 14 min and let to sit for another 20 min in the hot buffer. The
slides were then washed in tap water for 1 min. A ring was drawn round the tissue,
cellblock or cells with a liquid repellent marker pen. 3% hydrogen peroxide in methanol
(App. 5.9) was added to the slides for 5 min then washed with PBS (App. 5.9) for 5 min.
The slides were covered with 100µL of normal horse serum (1:100) (App. 5.9) for 5 min
then drained and primary antibody was added, NPC 1 or NPC 2 for 1h, 100µL on each
slide. The dilutions 1:50, 1:100, 1:150 and 1:200 were tried out. Slides were washed with
PBS for 3x2 min. Biotinylated secondary antibody (App. 5.9) was added to the slides,
100µL, for 15 min and then washed in PBS for 3x2 min. ABC (App. 5.9) was then added,
100µL, for 15 min and after that washed with PBS 3x2 min. DAB (diaminobenzidine) with
30% hydrogen peroxide (App. 5.9) was added to the slides for 7 min then washed in tap
water 1 min. The slides were then put in Mayer´s Haematoxylin for 40-60sec then blued in
warm tap water for 3 min. Slides were then dehydrated through spirit, absolute alcohol ad
xylene and then mounted in DPX.
22
3. RESULT
3.1 Sudan Black B
The Sudan Black B is a lipid and cholesterol stain. It was performed on frozen rat adrenal
(Fig.3.1) and acetone fixed U18666A treated HepG2 cells. To enhance the stain 2.5%
aqueous bromine was used thus the slides stained without it showed very poor stain. The
nuclei were stained with 0.2% Neutral Red but this was unsuccessful. The cytospin slides
with U18666A treated HepG2 cells were fixed in 10% formalin, pretreated with 2.5%
aqueous bromine and then stained with Sudan Black B. No lipid or cholesterol was stained
in this experiment.
Figure 3.1 Sudan Black B method on frozen rat adrenal.
3.2 Oil Red O
Oil Red O is a general hydrophobic lipid stain and was performed on frozen rat adrenal
(Fig. 3.2) and 10% formalin fixed U18666A treated HepG2 cells. The Oil Red O stain on
the frozen rat adrenal was successfully done. It showed beautiful red colour for the places
of lipids. The nuclei were stained with Mayer´s Haematoxylin for 30sec and that was
enough to view the morphology of it and get perspective of the tissue towards the lipid
stain. No staining was detected in the cells.
Figure 3.2 Oil Red O method on frozen rat adrenal. Nuclei stained with Mayer´s
Haematoxylin.
23
3.3 Filipin stain
The fluorescence method Filipin is used to visualize free cholesterol and is often used in
connection with Niemann-Pick type C disease. Filipin stain was performed on frozen rat
adrenal fixed in 3% formalin (Fig. 3.3.A) and U18666A treated HepG2 cells fixed in 3%
formalin (Fig. 3.3.B). The concentration used with Filipin was 250µg/mL.
Propidium Iodide with concentration 1mg/mL for nuclei stain was optimized on HeLa
cells fixed in 3% formalin (Fig. 3.3.C). The first staining performed was made with a
dilution of 1:500 for 10 min on rat adrenal and proved to be a much too strong staining.
Different dilutions and times were tried out as followed: 1:1000 for 5 min, 1:1000 for 10
min, 1:2000 for 10 min and 1:3000 for 10 min. The cells were fixed in 3% formalin before
staining. The dilution 1:1000 showed good nuclei staining and 5 min was enough for
exposure. A combined picture of Filipin and Propidium Iodide stain on HepG2 cells is
shown in Fig. 3.3.D and 3.3.E.
Figure 3.3.A Filipin stain on frozen rat adrenal.
Figure 3.3.B Filipin stain on HepG2 cells.
24
Figure 3.3.C Propidium Iodide nuclei stain on HeLa cells.
Figures 3.3.D and 3.3.E Combined Filipin and Propidium Iodide stain on HepG2 cells
with magnification 200x respective 400x.
25
3.4 Immunoperoxidase staining for NPC 1 and NPC 2 proteins
3.4.1 Normal and diseased tissues
The right dilution of antibodies and right unmasking method was established on paraffin
embedded tissues and then applied to cellblocks and cytospins with HeLa and U18666A
treated HepG2 cells.
NPC 2 was highly expressed in neurons and astrocytes in Alzheimer disease (Fig.
3.4.C.i and 3.4.C.ii) and neurons in healthy brain tissue (Fig. 3.4.F). NPC 2 was positive in
seminiferous tubules in testis (Fig. 3.4.B.i) but negative for NPC 1(Fig. 3.4.B.ii). Adrenal
was positive for NPC 2 (Fig. 3.4.A.i) but negative for NPC 1(Fig. 3.4.A.ii). Intestinal
tissue stained positive for neurons with NPC 2 but as for NPC 1the staining was negative
(Fig. 3.4.D.i and 3.4.D.ii). Epithelium in stomach tissue stained positive with both NPC 1
and NPC 2 (Fig. 3.4.Gi and 3.4.G.ii). In ovary tissue NPC 1 was highly expressed (Fig.
3.4.E) but according to Human Protein Atlas (www.proteinatlas.org) NPC 2 is not well
expressed in ovary tissue and therefore never used.
In rat tissue NPC 1 was positively expressed in kidney, liver and brain. (Fig. 3.4.H.i,
3.4.H.ii and 3.4.H.iii). In the rat brain though there was a weaker positive stain in neurons.
Antigen unmasking methods used were EDTA buffer, 10mM, with pH 8 (App. 5.9) and
Citrate buffer, 1mM, with pH 6 (App. 5.9). EDTA buffer with pH 8 was used for the
tissues stained with the NPC 1 antibody and Citrate buffer with pH 6 was used for the
tissues stained with the NPC 2 antibody.
Figures 3.4.A.i and 3.4.A.ii Immunoperoxidase staining for NPC protein in adrenal tissue.
Figure 3.4.A.i Positive NPC 2 and figure 3.4.A.ii Negative NPC 1.
26
Figure 3.4.B.i and 3.4.B.ii Immunoperoxidase staining for NPC protein in seminiferous
tubules in testis. Figure 3.4.B.i Positive NPC 2 and figure 3.4.B.ii Negative NPC 1.
Figure 3.4.C.i and 3.4.C.ii Immunoperoxidase staining for NPC protein in Alzheimer’s
disease. Figure 3.4.C.i Positive stain with NPC 2 for astrocytes and figure 3.4.C.ii Positive
stain with NPC 2 for neurons.
Figure 3.4.D.i and 3.4.D.ii Immunoperoxidase staining for NPC protein in intestine.
Figure 3.4.D.i Positive stain with NPC 2 for neurons and figure 3.4.D.ii Negative NPC 1.
27
Figure 3.4.E and 3.4.F Immunoperoxidase staining for NPC protein in ovary tissue and
brain. Figure 3.4.E Positive NPC 1and figure 3.4.F Positive NPC 2.
Figures 3.4.G.i and 3.4.G.ii Immunoperoxidase staining for NPC protein in epithelium in
stomach tissue. Figure 3.4.G.i Positive NPC 1 and Figure 3.4.G.ii Positive NPC 2.
Figures 3.4.H.i, 3.4.H.ii and 3.4.H.iii Immunoperoxidase staining for NPC protein in rat
tissue. Figure 3.4.H.i Positive NPC 1 in rat kidney, figure 3.4.H.ii Positive NPC 1 in rat
liver and figure 3.4.H.iii Weak positive stain with NPC 1for neurons in rat brain.
28
3.4.2 HepG2 and HeLa cells
The HeLa cells stained positive for both NPC 1 and NPC 2 (Fig. 3.4.I.i and 3.4.I.ii).
The results regarding the U18666A treated HepG2 cells there were varied result between
the HepG2 in cellblocks and those on cytospins. In the DMSO control for cellblocks, NPC
1 protein was detected (Table 3.4.A). HepG2 cells treated with U18666A were positive in
all concentrations and distinguished differences could not be detected between NPC 1 and
NPC 2 (Table 3.4.A). Stronger staining though was seen in HepG2 cells with 1.2µg/mL
U18666A than the others (Fig. 3.4.L.i and 3.4.L.ii).
Figures 3.4.I.i and 3.4.I.ii Immunoperoxidase staining for NPC protein in HeLa cells.
Figure 3.4.I.i Positive NPC 1 and figure 3.4.I.ii Positive NPC 2.
Table 3.4.A Results of evaluation of effects of U18666A on HepG2 cells in cellblocks.
NPC 1 NPC 2
5µL DMSO + -
5µL DMSO + 0.2µg/mL U18666A ++ ++
5µL DMSO + 0.4µg/mL U18666A +++ ++
5µL DMSO + 0.8µg/mL U18666A ++ +++
5µL DMSO + 1.2µg/mL U18666A +++ +++
29
Figures 3.4.J.i and 3.4.J.ii Immunoperoxidase staining for NPC protein in HepG2 cells
with DMSO. Figure 3.4.J.i Some positive stain with NPC 1 and figure 3.4.J.ii Negative
NPC 2.
Figures 3.4.K.i and 3.4.K.ii Immunoperoxidase staining for NPC protein in HepG2 cells
with 0.2µg/mL U18666A. Figure 3.4.K.i Positive NPC 1 and figure 3.4.K.ii Positive NPC
2.
Figures 3.4.L.i and 3.4.L.ii Immunoperoxidase staining for NPC protein in HepG2 cells
with 1.2µg/mL U18666A.Figure 3.4.L.i Positive NPC 1 and figure 3.4.L.ii Positive NPC 2.
30
Regarding the acetone fixed U18666A treated HepG2 cells on cytospins (Table 3.4.B) no
clear staining could be detected. Some staining was detected in one of the slides but cannot
single handedly be a result of positive staining (Fig. 3.4.M).
Table 3.4.B Results of evaluation of effects of U18666A on acetone fixed HepG2 cells on
cytospins.
NPC 1 NPC 2
5µL DMSO - -
5µL DMSO + 0.2µg/mL U18666A - -
5µL DMSO + 0.4µg/mL U18666A - -
5µL DMSO + 0.8µg/mL U18666A - -
5µL DMSO + 1.2µg/mL U18666A - -
Figure 3.4.M Focal positive immunoperoxidase staining for NPC 1protein in HepG2 cells
with 0.2µg/mL U18666A.
31
4. DISCUSSION
4.1 Sudan Black B and Oil Red O
Staining with Sudan Black B on the frozen rat adrenal was successful using 2.5% aqueous
bromine for 30 min as pretreatment. Without the 2.5% aqueous bromine pretreatment the
stain was very poor indicating that the lipid staining was cholesterol and cholesterol esters.
The nuclei stain with 0.2% Neutral Red was unfortunately unsuccessful as a nuclear stain.
The time used for nuclei stain was 3 min and a longer time than that should be tried out for
best result if using the concentration 0.2%.
Staining of the U18666A treated HepG2 cells for lipids did not induce lipid deposits in
the cells. This was noted using the Sudan Black B method and the Oil Red O method.
After cytospin preparation the cells were air dried and wrapped in tin foil before put in the
freezer unfixed and then before staining fixed in 10% formalin for 5 min. This fixation on
the cells may have affected the lipid stain and other fixation methods should be tried out.
Fixation with 4% buffered paraformaldehyde has been performed in a study using the Oil
Red O method which gave positive lipid stain (Rizk et al., 2004) and 50% ethanol was
used as fixation in a study regarding the Sudan Black B method (Travers et al., 2008).
The nuclei stain on the other hand using the 0.2% Neutral Red in the Sudan Black B
method on cells was positive. Time with 0.2% Neutral Red on the cells was on for 6 min
this time and gave good result. Same time can be a suggestion to use on the tissues as well
since 3 min is not enough.
4.2 Filipin stain
The fluorescence method Filipin is used to visualize free cholesterol and is often used in
connection with Niemann-Pick type C disease. The Filipin used was Filipin III from
Streptomyces filipinensis with the concentration 250µg/mL.
The Filipin stain was performed on frozen rat adrenal tissue and U18666A treated
HepG2 cells. Both the frozen rat adrenal and the HepG2 cells were fixed in 3% formalin
for 10 min before staining. The concentration of Filipin III, 250µg/mL, gave a good
staining on both the rat adrenal and the HepG2 cells.
Optimization for the fixation time in 3% formalin was also performed. For the first
staining with Filipin on this project the slides were fixed in 3% formalin for 30 min. For
32
the optimization of the fixation three slides with HeLa cells were used. One slide was fixed
with 3% formalin for 10 min, one slide for 30 min and one slide without the formalin
fixation. The slide without the formalin fixation gave no positive staining for free
cholesterol. The slides with formalin gave no difference in result due to time exposure so
therefore 10 min was used for the rest of the staining performed during the project
regarding the Filipin stain.
Differences in staining in the HepG2 cells could not be detected due to the different
concentrations of U18666A added to the cells. The concentrations and the range of
concentrations might have been too small to see any differences in the staining. In a study
from 1999 they used U18666A in the concentrations 0.01µg/mL and 0.1µg/mL with
Filipin staining on SK-N-SH cells, a human neuroblastoma cell line, which showed clear
differences in staining due to the U18666A concentrations (Sparrow et al., 1999).
4.3 Immunoperoxidase staining
The optimal dilution of antibodies and heat-based unmasking method was performed on
several formalin fixed, paraffin embedded human and rat tissues and then applied to
cellblocks and cytospins of HeLa and U18666A treated HepG2 cells. The best dilution
regarding the NPC 1 antibody was to be found 1:150 and had the least unspecific
background staining but still strong positive staining. In other studies, dilutions of NPC 1
antibody used were 1:100 combined with fluorescence (Falk et al., 1999) and 1:500 for
immunoperoxidase staining for localization of murine Niemann-Pick type C protein
(Garver et al., 2000).
Best antigen unmasking method for NPC 1 protein was using EDTA buffer with pH 8.
For the cellblocks the buffer was preheated for 10 min before putting the slides in and let
to sit for 20 min. This was performed because the cellblock sections had more tendencies
to fall off the slides. For the cellblock sections SuperFrost®
Plus microscope slides (VWR)
are recommended as adhesion was a problem.
For the NPC 2 protein the best dilution of the NPC 2 antibody was 1:100. In a study
done recently they used a dilution of 1:750 in mouse ovary with positive result (Busso et
al., 2010). For the NPC 2, Citrate buffer with pH 6 worked well as unmasking method.
Immunostaining requirements were similar for the cellblock as for the NPC 1, the Citrate
buffer was preheated for 10 min and then the slides were put in and let to sit for 20 min.
U18666A was added to HepG2 cells which causes cholesterol to accumulate. U18666A
33
is a cell permeable amphiphilic amino steroid that inhibits the intracellular biosynthesis
and transport of cholesterol (www.merck-chemicals.com). It decreases the cholesterol
content in the endoplasmic reticulum and impedes the cholesterol transport between the
lysosomal compartment and plasma membrane (Koh & Cheung, 2006) making it similar to
what happens in Niemann-Pick type C disease.
The optimized dilutions of the NPC 1 and NPC 2 antibodies were then tried out on HeLa
cells and the U18666A treated HepG2 cells with the concentrations 0.2µg/mL, 0.4µg/mL,
0.8µg/mL and 1.2µg/mL to see if there were any differences to be seen in the accumulation
of cholesterol in the cells relative to the concentrations of U18666A. Differences between
the NPC 1 and NPC 2 protein expression in the cell, due to the triggering of cholesterol
accumulation, were also to be investigated. No specific differences in NPC protein
expression could be detected though due to the concentrations of U18666A regarding the
cellblocks. The range between the concentrations may have been too small to view any
direct differences and the concentrations per se were too low and needs to be higher. In
other studies 2µg/mL of U18666A (Di Nunzio et al., 2010) has been used in HepG2 cells
which increased the staining. Cortical neurons from mice have been treated with U18666A
with a span over 0.1µg/mL to 50µg/mL which affected the lysosome enzymes cathepsins B
and D (Amritraj et al., 2009). CHO-K1 cells, an ovary cell line from hamster, were used in
a study treated with U18666A with concentrations 0.5µg/mL and 2µg/mL (Ridgway et al.,
1998) and showed stronger staining with 2µg/mL towards 0.5µg/mL.
As for the U18666A treated HepG2 cells on cytospins there were unsuccessful staining
for the NPC 1 and NPC 2 protein. After the cytospin preparation they were air dried and
then fixed in acetone for 5 min, air dried and wrapped in tin foil before freeze. Before
staining they were taken from the freezer, air dried and fixed in acetone again for 5 min.
The acetone fixation had adverse effects on the antigen and other fixations need to be
investigated. In another study, fixation by ethanol, ethanol/acetic acid and
paraformaldehyde/ethanol (Maciorowski et al., 1997) were used and
paraformaldehyde/ethanol fixation seemed to preserve antigen best.
HeLa cells in cellblocks stained positive for both the NPC 1 and the NPC 2 protein.
The Human Protein Atlas (www.proteinatlas.org) lists other cell lines that have high
expression of the NPC 1 and NPC 2 protein for example HMC-1, human mast cell; U-
138MG, a glioma cell line from the brain; U-2197, a sarcoma cell line and AN3-CA which
is a human endometrial cancer cell line.
34
4.4 Conclusion
For a good Sudan Black B stain 2.5% aqueous bromine as pretreatment is required.
Regarding the nuclei stain with 0.2% Neutral Red on tissues it needs to be improved.
Different kind of fixation of the cells needs to be tried out thus the acetone fixation did
not work for positive immunoperoxidase staining. The 10% formalin fixation for the lipid
dyes also need evaluation regarding to cell staining.
A larger range of concentrations of U18666A needs to be tried out for the accumulation
of cholesterol in HepG2 cells as well as higher concentrations to be able to better see any
differences between the expressions of the NPC 1 and NPC 2 proteins.
In this present study methods were optimized for evaluation of lipids, cholesterol and
NPC proteins in human and animal tissues. These will be used in study of neurological
diseases and in vitro studies of the effects of pharmaceutical agents (e.g. U18666A) on
cholesterol and NPC protein expression.
35
5. APPENDICES
5.1 Haematoxylin and Eosin – paraffin sections
1. Dewax (xylene x 2, absolute alcohol x 2, spirit, water)
2. Harris´s Haematoxylin 5 min
3. Wash in running warm water to blue sections 3min
4. Differentiate in 1% Acid-alcohol 2sec
5. Blue in warm tap water 3 min
6. Stain in 1% Eosin
7. Rinse well with tap water
8. Dip in spirit 3 times then absolute alcohol x 2, xylene x 2
9. Mount in DPX
5.1.1 Material H & E-stain – paraffin sections
1% Eosin – 1g Eosin, Merck + 100mL dH2O
1% acid-alcohol – 1400mL absolute alcohol + 600mL dH2O → 20mL + 20mL HCl
Absolute alcohol
DPX, BDH
Harris´s Haematoxylin
Spirit
Xylene, 95% industrial methylated spirit
5.2 Haematoxylin and Eosin stain – frozen sections
1. Fix sections in 2% Acetic-Alcohol 10min
2. Rinse in tap water
3. Stain with Harris Haematoxylin 2 min
4. Rinse by dipping in a bath of tap water
5. 1% acid-alcohol for 1 sec then place slide back in tap water immediately
6. Blue in warm tap water 5 min
7. Counterstain with 1% Eosin 3 min
8. Rinse in tap water
9. Dehydrate, clear and mount in DPX
36
5.2.1 Material H&E-stain – frozen sections
1% Eosin – 1g Eosin, Merck + 100mL dH2O
1% acid-alcohol – 1400mL absolute alcohol + 600mL dH2O → 20mL + 20mL HCl
2% acetic-alcohol – 2mL 100% acetic-acid + 98mL absolute alcohol
Absolute alcohol
DPX, BDH
Harris Haematoxylin
Spirit
Xylene, 95% industrial methylated spirit
5.3 Cell culture
Foetal calf serum, 500mL Sigma Lot. 017K3395
Glutamine 200mmol, Gibco Lot. 709212
HeLa cells
HepG2 cells
PIS (10000 units/mL penicillin/10000 mg/mL streptomycin), Gibco Lot. 1359297
RPMI-1640 Medium 500mL, Sigma Lot. RNBB1150
Sterile universal container 20mL, Greiner bio-one Lot. 091523
Tissue culture flask 25cm2, Sarstedt Lot. 831810
Tissue culture flaks 75cm2, Greiner bio-one Lot. 09200142
5.4.i Harvesting – HeLa cells
EDTA/PBS – 0.2g EDTA (ethylenediaminetetracetic acid), Sigma + 1000mL PBS
PBS (phosphate buffered saline) 1 tablet/100mL dH2O, Oxoid Lot. BR0014G
RPMI Medium with Foetal calf serum, Glutamine and PIS
Sterile universal container 20mL, Greiner bio-one Lot. 091523
Tissue culture flasks 75cm2, Greiner bio-one Lot. 09200142
Trypsin – 50mL of 2.5% stock, Gibco + 500mL earles balanced salts, Sigma
5.4.ii HepG2 cells – Exposure to U18666A experiment
DMSO (dimethyl sulphoxide), Sigma Lot. 123H08711
EDTA/PBS – 0,2g EDTA (ethylenediaminetetracetic acid ), Sigma + 1000mL PBS
37
PBS (phosphate buffered saline) 1 tablet/100mL dH2O, Oxoid Lot. BR0014G
RPMI Medium with Foetal calf serum, Glutamine and PIS
Sterile universal container 20mL, Greiner bio-one Lot. 091523
Tissue culture flasks 75cm2, Greiner bio-one Lot. 09200142
Trypsin – 50mL of 2,5% stock, Gibco + 500mL earles balanced salts, Sigma
U18666A 100µg/mL – 20µL of U18666A 5mg/mL stock solution (5mg U18666A
+ 1mL DMSO), Sigma + 1mL RPMI medium, Sigma
5.5 Cellblock preparation
10% Formalin – 10mL conc. formalin + 90mL dH2O
2% Agar (bacteriological agar, no salts added) – 1g agar + 50mL dH2O
Cassette
EDTA/PBS – 0,2g EDTA (ethylenediaminetetracetic acid), Sigma + 1000mL PBS
Knife
Lid
PBS (phosphate buffered saline) 1 tablet/100mL dH2O, Oxoid Lot. BR0014G
RPMI Medium with Foetal calf serum, Glutamine and PIS
Sterile universal container 20mL, Greiner bio-one Lot. 091523
Trypsin – 50mL of 2.5% stock, Gibco + 500mL earles balanced salts, Sigma
5.6 Sudan Black B protocol
0.2% Neutral Red – 0.2g Neutral Red stock solution, BDH Lot. 34056 4A + 100mL
dH2O
0.5% Sodium metabisulphite – 0.5g sodium metabisulphite, BDH Chemicals +
100mL dH2O
2.5% Aqueous bromine – 2.5g bromine + 100mL dH2O
70% Ethanol – 70mL ethanol + 30mL distilled water
Glycerine jelly – 10g gelatine + 60mL dH2O + 70mL glycerol
Sudan Black B working solution – 1.5g Sudan Black B stock solution, Gurr +
100mL 70% ethanol
38
5.7 Oil Red O protocol
10% Formalin – 10mL conc. formalin + 90mL dH2O
60% Isopropanol – 60mL isopropanol + 40mL dH2O
Glycerine jelly – 10g gelatine + 60mL dH2O + 70mL glycerol
Mayer’s Haematoxylin
Oil Red O working solution – 30mL Oil Red O stock solution, Gurr + 20mL dH2O
5.8 Filipin stain
1.5mg/mL glycine in PBS – 1.5g glycine + 100mL PBS
3% Formalin – 3mL conc. formalin + 97mL dH2O
DMSO (dimethyl sulphoxide), Sigma Lot. 123H08711
Filipin 250µg/mL – 1µL Filipin stock 25mg/mL (40µL DMSO + 1mg Filipin),
Sigma + 99µL PBS
Glycerol in PBS – 1drop glycerol + 9 drops PBS
PBS (phosphate buffered saline) – 1tablet/100mL dH2O
Propidium Iodide 1mg/mL, Fluka Lot. 1167235
5.9 Immunoperoxidase staining
2M NaOH – 80g NaOH, BDH + 1000mL dH2O
3% Hydrogen peroxide – 1mL 30% hydrogen peroxide, VWR + 9mL methanol
Absolute alcohol
APES (3-aminopropyltriethoxysilane) microscope slides, Knittel Glass
Citrate buffer pH 6 – 2.1g Citrate, Merck + 1000mL dH2O, pH to 6 with 2M NaOH
DAB (diaminobenzidine), Sigma – frozen DAB aliquots 0.2 mL+ 1.8mL PBS +
10µL 30% hydrogen peroxide
DPX, BDH
EDTA buffer pH 8 – 3.7g EDTA (ethylenediaminetetracetic acid), Sigma +
1000mL distilled water, pH to 8 with 2M NaOH
Liquid Blocker, liquid repellent slide marker pen
Mayer’s Haematoxylin
PBS (phosphate buffered saline) 1 tablet/100mL dH2O Oxoid Lot. BR0014G
Primary antibody, anti-NPC 1 and anti-NPC 2, Sigma Lot. R12288, R00021
39
Spirit
SuperFrost® Plus microscope slides, VWR Lot. 12499
Vectastain ABC kit, Vector Laboratories Lot. 271 210:
- Biotinylated secondary antibody – two drops of stock solution + two drops of
normal horse serum stock solution + 5mL PBS
- Normal horse serum – one drop of stock solution + 5mL PBS
- Vectastain Elite® ABC reagent – two drops each of stock solutions A and B +
5mL PBS
Xylene, 95% industrial methylated spirit
40
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